Study site

We used fossils from Hall's Cave in the Edwards Plateau, Texas (Fig. 1B). This site is a fluvial deposit with episodic deposition of sediments and biological materials following heightened periods of precipitation (Toomey, Reference Toomey1993). The Hall's Cave record extends back to ca. 20,000 cal yr BP, with an exceptionally well-dated stratigraphic sequence (Fig. 1C). Excavations from Hall's Cave began in the 1960s and accelerated in the late 1980s–1990s (Toomey, Reference Toomey1993). To date, the site has yielded thousands of vertebrate specimens, particularly of small and medium body sizes across various trophic guilds (Toomey, Reference Toomey1993). The vertebrate fossils are housed at the Vertebrate Paleontology Lab of the Texas Memorial Museum (TMM) at the University of Texas, Austin.

Study organisms

Three Neotoma species are hypothesized to be present in the Hall's Cave fossil record: N. albigula, N. floridana, and N. micropus (Toomey, Reference Toomey1993), with the latter two extant on the Edward's Plateau today (Fig. 1A). Unfortunately, the three species cannot be distinguished based solely on molar or lower-jaw characteristics (Sagebiel, Reference Sagebiel2010; Tomé et al., Reference Tomé, Whiteman-Jennings and Smith2020b), which represent the vast majority of our fossil elements. Moreover, there is substantial body size overlap among the species. Thus, we aggregated samples and asked questions at the level of the genus, which we note is common for paleoecological studies. Nonetheless, we note that preliminary ancient DNA work conducted on a sediment column taken from Hall's Cave suggested a high probability that Neotoma floridana is the only woodrat present in the oldest (prior to the extinction boundary at ca. 13,000 cal yr BP) stratigraphic levels (Seersholm et al., Reference Seersholm, Werndly, Grealy, Johnson, Keenan Early, Lundelius and Winsborough2020).

Neotoma fossils are present in all strata at Hall's Cave from ca. 22,000 cal yr BP to modern deposits (Toomey, Reference Toomey1993); however, specimen abundance varies by stratum. To facilitate our analyses of body size and diet of Neotoma over time, we aggregated data into 15 time intervals of approximately equal length, chosen and accounting for important environmental transitions (Table 1). Note that the oldest time interval is longer, spanning 22,400–15,800 cal yr BP; this is because Neotoma fossil bones were rare, with only 31 elements recovered in this interval. Thus, to increase sample size, we also included a sample of 14 additional Neotoma specimens from Zesch Cave, a nearby fossil site, ~75 km away, at 470 m in elevation, and dating to 18,000–16,000 cal yr BP (Lundelius, Reference Lundelius, Martin and Wright1967; Graham et al., Reference Graham, Graham, Semken and Graham1987; Sagebiel, Reference Sagebiel2010). The Zesch Cave record shares a similar community composition to that of Hall's Cave, including the same three potential Neotoma species. To verify that climatic regimes at this time were similar between Zesch Cave and Hall's Cave (~680 m elevation), we compared climate data from the Community Climate System Model (Lorenz et al., Reference Lorenz, Nieto-Lugilde, Blois, Fitzpatrick and Williams2016a, Reference Lorenz, Nieto-Lugilde, Blois, Fitzpatrick and Williamsb). We found that mean annual precipitation, maximum temperature, and minimum temperature differed by ~32.5 mm, ~7.1°C, and 4.7°C, respectively, between the two sites, with temperature differences falling within one standard deviation for the time bin spanning 22,400–15,800 cal yr BP. Two sample t-tests found no significant difference in body size or bone collagen δ¹³C and δ¹⁵N values of Neotoma from Zesch Cave and Hall's Cave (Supplementary Table S1). All other (i.e., younger) time bins include only specimens from Hall's Cave.

Table 1. Summary of data for Neotoma by time interval. Precipitation, maximum and minimum temperature were extracted from the CCM3 (Lorenz et al., Reference Lorenz, Nieto-Lugilde, Blois, Fitzpatrick and Williams2016a, Reference Lorenz, Nieto-Lugilde, Blois, Fitzpatrick and Williamsb) in 500 year intervals and average each time interval given below. Sorenson to Modern is the Sorenson Index calculated in terms of similarity to the community composition of the youngest time interval (0–1500 cal BP).

Morphology

We estimated body size in Neotoma using linear measurements of the first upper (UM1) and lower molars (LM1). These molars were either loose or found in mandibular or maxillary elements, generally with incomplete toothrows. The upper or lower M1 of 693 Neotoma fossils were photographed using a calibrated AM4515ZT Dino-Lite Edge digital microscope. The length of each molar was measured three times (~2080 measurements) using the line tool in DinoCapture 2.0. Samples that could not be well characterized or whose measurements resulted in a >5% standard error were discarded, which led to the elimination of 22 specimens. We calculated the minimum number of individuals (MNI) to exclude potentially replicated individuals because it was not possible to determine whether loose molars were definitively from different specimens or potentially from different quadrants (upper right and left, and lower right and left) from the same individual.

To help in the estimation of MNI, we determined the ‘normal’ asymmetry of teeth found among modern woodrats. By measuring all the first molars (upper and lower, right and left) for a total of 20 museum specimens, which included individuals from the species Neotoma floridana and N. albigula from the Museum of Southwestern Biology (MSB) at the University of New Mexico (Albuquerque, NM) and the James F. Bell Museum of Natural History (MMNH) at the University of Minnesota (St. Paul, MN) (Supplementary Table S2), we characterized the upper versus lower and bilateral symmetry of woodrat teeth. We found that on average, upper first molars (UM1) were ~5% larger than lower first molars (LM1). Moreover, bilateral symmetry was high, with only an average difference of ~0.5% between left and right measurements. These results were independent of species and provided a strategy for analysis: using 0.5% as a cutoff we were able to determine whether loose molars from a stratum could realistically belong to different Neotoma. First, we preferentially selected only lower left first molars (LLM1s) for each stratigraphic level. Second, we then included all lower right first molars (LRM1s) from that level that were 0.5% greater or smaller in size than any measured LLM1s in the sample. Third, after standardizing the size of upper molars to that of lower molars with a 5% length reduction, we included upper left first molars (ULM1s) from that level that were 0.5% greater or smaller in size than any lower molars selected in the first two steps. Lastly, we included upper right first molars (URM1s) from the same level that were 0.5% greater or smaller in size than any previously selected LLM1s, LRM1s, and ULM1s. Thus, we ensured that separately measured elements were not from the same individual within a stratum.

Tooth measurements were translated into estimates of body mass using an allometric equation for cricetid rodents for the first lower molar length (Martin, Reference Martin, Damuth and MacFadden1990):

$${\rm Log\ mass\ }( {\rm g} ) = 3{\rm .310 \, \ast \,}( {{\rm Log\ LM1\ length}} ) + 0{\rm .611\ }( {{\rm r}^ 2 = 0{\rm .96, \;\ \% PE\ } = 15{\rm .58, \;\ df\ } = 32} ) $$

To account for differences between lower and upper molar length in Neotoma, upper molar length was standardized by a 5% decrease to measurements prior to calculating body mass. After the removal of potential duplicates, our final dataset included body mass estimates for 430 individual Neotoma across the 15 levels, including mass estimates for 10–63 individuals per time bin (Table 1).

Isotope-based estimates of diet composition and variation

We used stable isotope analysis to characterize shifts in diet for Neotoma across time. We measured carbon (δ¹³C) and nitrogen (δ¹⁵N) isotope values of bone collagen extracted from maxillary and mandible bones for 367 Neotoma fossils. We attempted to acquire 10 or more samples per time interval; however, sparsity of material led to some intervals containing fewer than 10 individuals, and we excluded a single interval that only contained five individuals (22,400–15,800 cal yr BP). Differences in how plants that use the C₃ versus C₄ photosynthetic pathway fractionate carbon isotopes leads to natural variation in δ¹³C values across ecosystems and are reflected in the tissues of consumers that utilize these resources (DeNiro and Epstein, Reference DeNiro and Epstein1978; Farquhar et al., Reference Farquhar, Ehleringer and Hubick1989; Cerling et al., Reference Cerling, Harris, MacFadden, Leakey, Quade, Eisenmann and Ehleringer1997). Regional studies in the Great Plains and southern/central Texas have found that C₃ and C₄ plants have mean (±SD) δ¹³C values of about -27 ± 5‰ and -13 ± 4‰, respectively (Boutton et al., Reference Boutton, Nordt, Archer, Midwood and Casar1993, Reference Boutton, Archer, Midwood, Zitzer and Bol1998; Derner et al., Reference Derner, Boutton and Briske2006). δ¹⁵N values of consumers reflect a combination of trophic position and/or shifts in the baseline nitrogen isotope composition of primary producers, with higher δ¹⁵N values signifying higher trophic position or increased aridity (DeNiro and Epstein, Reference DeNiro and Epstein1981; Ambrose, Reference Ambrose1991; Amundson et al., Reference Amundson, Austin, Schuur, Yoo, Matzek, Kendall, Uebersax, Brenner and Baisden2003). Consumer tissue δ¹³C and δ¹⁵N values systematically differ from that of their diet due to physiologically mediated isotopic discrimination (Koch, Reference Koch, Michener and Lajtha2007) and these differences are quantified as trophic discrimination factors (TDF). Thus, at a particular time interval, δ¹³C and δ¹⁵N values vary across animals in a community depending upon their trophic level and the relative proportion of C₃ versus C₄ vegetation in their diet, which allows for use of isotopic niche space of small mammals that do not move large distance as a proxy for dietary niche space (Newsome et al., Reference Newsome, Martinez del Rio, Bearhop and Phillips2007).

A subsample of ~150–250 mg of bone was collected from each fossil mandible or maxilla using a low-speed Dremel tool. To extract collagen, we demineralized samples with 0.25N HCl at 3–4°C for 24–48 hours. Samples were then lipid extracted via soaking in 2:1 chloroform/methanol for 72 hours, changing the solution every 24 hours. Each sample was then washed 5–7 times with distilled water and lyophilized. Approximately 0.9–1.0 mg of collagen was placed into 3 × 5 mm tin capsules. Collagen δ¹³C and δ¹⁵N values were measured with a Costech elemental analyzer (Valencia, CA) interfaced with a Thermo Scientific Delta V Plus isotope ratio mass spectrometer (Bremen, Germany) at the University of New Mexico Center for Stable Isotopes (Albuquerque, NM). Isotope values are reported as δ values, where δ = 1000[(R_sample/R_standard)-1] and R_samp and R_std are the ¹³C:¹²C or ¹⁵N:¹⁴N ratios of the sample and standard, respectively; units are in parts per thousand, or per mil (‰). Samples were calibrated using international reference standards; Vienna Pee Dee Belemnite (VPDB) for carbon, and atmospheric N₂ for nitrogen (Fry, Reference Fry2006; Sharp, Reference Sharp2017). Analytical precision was assessed via repeated within-run analysis of organic reference materials calibrated to international standards and was determined as ≤0.2‰ for both δ¹³C and δ¹⁵N values. We also measured the weight percent carbon and nitrogen concentration of each collagen sample. Mean (±SD) [C]:[N] ratios for Neotoma (N = 378) were 2.9 ± 0.14 and we excluded any samples from subsequent analyses whose [C]:[N] ratios were >3.5 (Ambrose, Reference Ambrose1990).

We followed our protocol for MNI as outlined above for the mass estimates to ensure that each sample chosen for isotope analysis represented a unique individual. Our final dataset for the isotopic analyses consisted of 306 individuals (Table 1). Not all specimens for which we had δ¹³C and δ¹⁵N measurements had body measurements, and vice versa. Of the 430 individuals with mass measurements and 306 with isotope measurements, 131 individuals had both.

Community, climate, and vegetation data

We compared our body-size and isotope data with measures of the mammal community composition and turnover, climate (temperature and precipitation), and several measures of vegetation composition and change. Community data included α-diversity (richness) and β-diversity (Sorenson Index) extracted from Smith et al. (Reference Smith, Tomé, Elliott Smith, Lyons, Newsome and Stafford2016b), updated to reflect current phylogeny and cave fossil assembly information, and recalculated to fit within the time intervals used here (Table 1). Here, we used the Sorenson Index to calculate turnover between adjacent time intervals and similarity to the modern community composition. Turnover, defined as similarity to the previous time interval, can be used to evaluate changes in species composition between time bins and provides information on whether the presence/absence of certain species may be affecting responses in Neotoma. Similarity to modern provides insight into whether species turnover is related to species permanently leaving the community and being replaced or leaving and re-entering the community through time. The original community data for Hall's Cave were compiled by Toomey (Reference Toomey1993) and expanded to encompass the Edwards Plateau using the Neotoma Paleoecology Database (2015) by Smith et al. (Reference Smith, Tomé, Elliott Smith, Lyons, Newsome and Stafford2016b).

Climate information was sourced from the Community Climate System Model (CCSM3), which simulates climate across North America for the past 21,000 years (Lorenz et al., Reference Lorenz, Nieto-Lugilde, Blois, Fitzpatrick and Williams2016a, Reference Lorenz, Nieto-Lugilde, Blois, Fitzpatrick and Williamsb). The CCSM3 data have 0.5° spatial resolution, so we were able to obtain regional-scale climate for the Edwards Plateau. Mean annual maximum and minimum temperature and total mean annual precipitation data were extracted from the CCSM3 at 500 year intervals. We averaged values to the same temporal intervals used for our fossil morphometric and isotopic data (Table 1; Fig. 2A–C).

Figure 2. Temporal changes in climate and vegetation on the Edwards Plateau, including (A) mean maximum temperature, (B) mean minimum temperature, and (C) mean annual precipitation (mm) (Lorenz et al., Reference Lorenz, Nieto-Lugilde, Blois, Fitzpatrick and Williams2016a, Reference Lorenz, Nieto-Lugilde, Blois, Fitzpatrick and Williamsb). (D) Pollen counts showing the relative abundance of C₃ versus C₄ (%) grasses (C₃ grasses/C₄ grasses × 100), Cupressaceae, and Opuntia at Hall's Cave over time (Cordova and Johnson Reference Cordova and Johnson2019).

We compared the Neotoma body-size and isotope data with a vegetation reconstruction from Hall's Cave based on phytolith and pollen data from 47 stratigraphic depths spanning the past 18,000 years (Cordova and Johnson, Reference Cordova and Johnson2019). The ratio of C₃ to C₄ grasses derived from phytolith data serves as an index for the prevalence of C₄ grasses on the landscape, with declining C₃:C₄ values during the Holocene reflecting a shift from forests dominated by C₃ plants to grasslands dominated by C₄ grasses in response to drier conditions (Cordova and Johnson, Reference Cordova and Johnson2019). Because modern Neotoma albigula, N. floridana, and N. micropus differ in their use of prickly pear cacti and juniper, we also compared our Neotoma data with changes in the relative abundance of Opuntia (prickly pear) and Cupressaceae (the family including juniper) pollen. Modern Neotoma albigula and N. micropus are known to consume prickly pear cacti, which can represent up to 45% of the annual diet of N. albigula (Vorhies and Taylor, Reference Vorhies and Taylor1940; Spencer and Spencer, Reference Spencer and Spencer1941; Macêdo and Mares, Reference Macêdo and Mares1988; Braun and Mares, Reference Braun and Mares1989). Moreover, N. albigula makes more use of juniper than either Neotoma floridana or Neotoma micropus (Rainey, Reference Rainey1956; Finley, Reference Finley1958; Wiley, Reference Wiley1980; Dial, Reference Dial1988; Schmidly and Bradley, Reference Schmidly and Bradley2016). We calculated mean values of C₃:C₄ grasses in the phytolith data and mean pollen percentages for Opuntia and Cupressaceae for each of our 15 time intervals (Fig. 2D).

Statistical analyses

We employed both parametric and non-parametric tests to examine changes in body mass and isotope values over time because in some instances our data violated assumptions of normality. All statistical analyses were performed using R software version R.3.6.0 (R Core Team, 2019) and RStudio 1.2.1335 (RStudio Team, 2019).

We first used an F-test and a Bartlett's test to assess changes in body mass and isotope variation before and after the extinction boundary (ca. 13,000 cal yr BP) to determine if there were marked changes associated with this period of acute biodiversity loss. To examine changes in mass across all 15 time intervals, we used ANOVA and Tukey multiple comparisons. Least squares linear regressions were also run using maximum (i.e., largest individual per time interval) and median mass against the mean δ¹³C, δ¹⁵N, climate, and community variables to evaluate their influence on body mass. When significant correlations were found, we conducted an analysis of covariance (ANCOVA) to assess the added effect of each on mass.

We characterized shifts in isotopic niche space using Bayesian-based standard ellipse areas (SEA_B) of δ¹³C and δ¹⁵N, and calculated the overlap of SEA_B between adjacent time intervals using the siberEllipses and maxLikOverlap functions from the SIBER package for R (Parnell and Jackson, Reference Parnell and Jackson2013; R Core Team, 2019). We used an ANOVA to assess whether changes in SEA_B were affected by sample size within time interval. The standard ellipses representing 50% of the datapoints for each time interval were plotted using JMP Pro 13 (version 13.1). Because exact trophic discrimination factors (TDFs) for Neotoma are not yet available, we used the SIDER package in R (Healy et al., Reference Healy, Guillerme, Kelly, Inger, Bearhop and Jackson2018) to calculate TDFs for Neotoma. The SIDER package uses a dataset of known Δ¹³C and Δ¹⁵N TDFs (Healy et al., Reference Healy, Guillerme, Kelly, Inger, Bearhop and Jackson2017), habitat information (e.g., terrestrial), consumer diet information (e.g., herbivore), and a phylogenetic regression model to estimate the TDFs for a particular tissue type (e.g., bone collagen) of mammal or bird species (Healy et al., Reference Healy, Guillerme, Kelly, Inger, Bearhop and Jackson2018). Using the SIDER package and dataset, we calculated the δ¹³C diet-collagen TDFs for Neotoma albigula (1.9‰), N. floridana (1.9‰), and N. micropus (1.8‰), and then applied a mean (±SD) TDF of ~1.9 ± 0.5‰ for Neotoma at Hall's Cave. We calculated the proportion of C₃ in the diet of Neotoma for each time interval by running a mixing model in MixSIAR (Stock and Semmens, Reference Stock and Semmens2016) using mean δ¹³C values for C₃ (-27‰) and C₄ (-13‰) vegetation (Boutton et al., Reference Boutton, Archer, Midwood, Zitzer and Bol1998; Derner et al., Reference Derner, Boutton and Briske2006) and the estimated TDF. Changes in isotopic niche space were tested by analyzing δ¹³C and δ¹⁵N values using ANOVA and Tukey multiple comparisons across 14 time intervals due to lack of sufficient sample size in the oldest interval. Least squares linear regressions were run using mean, minimum, and maximum δ¹³C and δ¹⁵N against maximum and median mass, as well as climate, vegetation, and community variables.

We used a sliding window approach to test whether climate (temperature or precipitation) or community (richness or turnover) had a stronger effect on Neotoma at different times from the late Pleistocene to present. The sliding window consisted of six time intervals, whose start and end intervals shifted by a single interval across each iteration, for a total of 10 windows to progress across our 15 previously designated time intervals. We ran least squares linear regressions using maximum and median mass against maximum and minimum temperature, mean precipitation, species richness, turnover, and similarity to modern to determine variation in the impact of each factor between windows. For the purposes of these analyses, we assume no turnover between the community composition previous to the time interval between 22,400–15,800 cal yr BP, such that we can include all 15 time intervals and we began with a baseline of 0 for turnover.